利用代谢组学研究大气细颗粒物的生殖毒性效应

大气细颗粒物(PM2.5)污染已成为严峻的环境问题,探究PM2.5的毒性效应和机理变得尤为重要.本研究利用基于液相色谱/质谱的代谢组学技术,分析经PM2.5悬混液气管滴注暴露后成年雄性大鼠睾丸代谢组的全局变化,采用偏最小二乘判别分析法和非参数检验进行统计分析.结果表明,PM2.5暴露组大鼠睾丸的油提和水提代谢指纹谱均可与对照组实现准确区分,表明PM2.5暴露对大鼠睾丸的整体代谢网络产生了显著影响,最终鉴定出56个差异代谢物.通路分析显示,PM2.5暴露会引起大鼠睾丸的氨基酸和核苷酸代谢紊乱、类固醇激素代谢失衡以及脂类代谢异常,而这些重要通路可能是PM2.5生殖毒性的关键分子事件.     

火焰原子吸收光谱法研究五种螯合剂对染镉小鼠睾丸中镉钙铁锌浓度的影响

采用火焰原子吸收光谱法分别对染镉小鼠和N-对羟甲苯甲基-D-葡糖二硫代氨基甲酸钠(HBGD)、N-苯甲基-D-葡糖二硫代氨基甲酸钠(BGD)、二乙基二硫代氨基甲酸钠(DDTC)、二巯基丙醇(BAL)、乙二胺四乙酸(EDTA)等五种螯合剂治疗组小鼠睾丸中镉、钙、铁、锌等金属浓度进行了测定和研究.结果表明:镉染毒(Cd 2.5 mg·kg-1,腹腔注射)后,小鼠睾丸中镉、钙、铁、锌等金属浓度显著高于对照组(p＜0.05),染镉30 min后用各螯合剂治疗(0.400 mmol·kg-1,腹腔注射),24 h后除EDTA外,其余螯合剂能明显降低睾丸中镉的浓度并抑制钙、铁、锌浓度的增加(p＜0.05);染镉24 h后注射各螯合剂,治疗24 h后,HBGD、BGD和DDTC显著降低了小鼠睾丸中各金属浓度(p＜0.05);提示HBGD和BGD有望成为染镉中毒的理想解毒剂.     

中国绿螂精巢的组织学研究

运用光镜技术研究了中国绿螂精巢的组织结构及精子的发生过程.结果显示,中国绿螂的精巢由外壁及其内的无数生殖小管构成.外壁含单层柱状上皮细胞以及较厚的肌肉层.生殖小管的外层为生殖上皮,并由生殖上皮不断向腔内增殖产生精原细胞、初级精母细胞、次级精母细胞、精细胞和精子.伴随着染色质的浓缩,精子发生过程中细胞逐渐变小.中国绿螂的精子呈细长锥体状,形似辣椒,长约8～10 μm.     

Cellular organisation of the mature testes and stages of spermiogenesis in Danio rerio (Cyprinidae; Teleostei)--structural and ultrastructural studies

The male gonads of Danio rerio occupy a position typical of the Teleostei species. The structure of the testes corresponds to the anastomosing tubular type with unrestricted spermatogonia and represents a cystic type of spermatogenesis. The results of this study indicate that four distinct stages of cell differentiation can be identified during spermiogenesis. These stages are characterised by chromatin condensation, the development of flagellum, nuclear rotation, the formation of nuclear fossa and the elimination of excess cytoplasm. A round head and the absence of an acrosome characterise the differentiated sperm. The midpiece is short and large, and C-shaped mitochondria form a ring surrounding the initial region of the flagellum. The axoneme shows a 9 + 2 pattern. In the D. rerio spermatozoa the flagellar axis is at an angle of 110° to the nucleus diameter running through the centriole.     

高功率微波辐照对雄性大鼠生殖细胞的影响

 采用激光扫描共聚焦显微镜观察受不同参数高功率微波辐照后的大鼠精子细胞内Ca²⁺的变化,同时观察了辐照后大鼠的生殖细胞微核率、畸形率、精子数量、存活率和顶体酶反应的变化。实验表明：此条件下的高功率微波辐照对雄性大鼠的生殖细胞微核率和畸形率没有明显的损伤效应,但4×10⁵次脉冲的高功率微波辐照对大鼠的顶体酶反应有较明显的抑制作用,可能通过改变细胞内第二信使的Ca²⁺浓度来影响其生殖细胞功能。     

稀土镧对雄性小鼠睾丸cAMP和自由基的影响

采用酶联免疫吸附法和分光光度法,通过腹腔注射不同剂量稀土镧,研究小鼠睾丸环磷腺苷(cAMP)和自由基水平的变化。在稀土镧作用下,与对照组相比,处理组小鼠睾丸cAMP含量显著降低(P<0.05);MDA含量显著升高(P<0.05);GSH-PX活力无显著变化(P<0.05)。400mg·kg-1·d-1剂量组睾丸SOD活力显著降低(P<0.05)。腹腔注射稀土镧导致小鼠睾丸cAMP含量和SOD活力降低,可能是导致小鼠精子质量下降的重要原因。     

1H magnetic resonance spectroscopy of the normal testis: preliminary findings

PURPOSE: The purpose of this study was to determine the pre- and postpubertal 1H magnetic resonance spectroscopic characteristics of the normal testis to establish baseline values for further clinical studies. MATERIALS AND METHODS: The subjects consisted of male volunteers, of whom 19 were prepubertal with ages between 7 and 13 years and 24 were postpubertal with ages between 19 and 39 years. Their testes were evaluated at 1.5 T with magnetic resonance spectroscopy; in addition, testis volumes were measured. Major metabolite peaks were identified and their ratios were calculated. Metabolite differences of testis between pre- and postpubertal age were analyzed. RESULTS: Major constituents of spectra were 3.21 ppm choline and 0.9-1.3 ppm lipid peaks. At the echo time (TE) spectrum of 31 ms, choline/lipid ratios ranged from 0.35 to 8.30 (mean=1.87) in postpubertal males and from 0.06 to 5.45 (mean=0.88) in prepubertal males (P<.013). At the TE spectrum of 136 ms, choline/lipid ratios ranged from 0.66 to 15.42 (mean=4.09) in postpubertal males and from 0.05 to 4.91 (mean=0.9) in prepubertal males (P<.016). CONCLUSIONS: Choline/lipid ratio was higher in the postpubertal period. The existence of higher choline peak in that age group should be due to the initiation of spermatogenesis. The decrease in the lipid peak may represent the effect of testosterone on testicular tissue or may be due to histochemical changes initiated by puberty. The significant decrease in choline/lipid ratio noted after puberty could represent the presence of spermatogenesis. This hypothesis should be evaluated by further studies on postpubertal subjects with impaired spermatogenesis.     

New application of a subcellular fractionation method to kidney and testis for the determination of conjugated linoleic acid in selected cell organelles of healthy and cancerous human tissues

To clarify the mechanism of the anticarcinogenic effect of conjugated linoleic acid (CLA), its intracellular distribution needs to be determined. Subcellular fractionation using centrifugation techniques is a method that is frequently used for isolation of cell organelles from different tissues. But as the size and density of the organelles differ, the method needs to be optimised for every type of tissue. The novelty of this study is the application of a subcellular fractionation method to human healthy and cancerous renal and testicular tissue. Separation of total tissue homogenate into nuclei, cytosol, and a mixture of mitochondria and plasma membranes was achieved by differential centrifugation. As mitochondria and plasma membranes seemed to be too similar in size and weight to be separated by differential centrifugation, discontinuous density-gradient centrifugation was carried out successfully. The purity of the subcellular fractions was checked by measuring the activity of marker enzymes. All fractions were highly enriched in their corresponding marker enzyme. However, the nuclear fractions of kidney and renal cell carcinoma were slightly contaminated with mitochondria and plasma membrane fractions of all tissues with lysosomes. The fraction designated the cytosolic fraction contained not only cytosol, but also microsomes and lysosomes. The CLA contents of the subcellular fractions were in the range 0.13–0.37% of total fatty acids and were lowest in the plasma membrane fractions of all types of tissue studied. C16:0, C18:0, C18:1 c9, C18:2 n-6, and C20:4 n-6 were found to be the major fatty acids in all the subcellular fractions studied. However, marked variations in fatty acid content between subcellular fractions and between types of tissue were detectable. Because of these differences between tissues, no general statement on characteristic fatty acid profiles of single subcellular fractions is possible.